AU675166B2 - Peptide having inflammation affinity and radioactive diagnostic containing the same - Google Patents
Peptide having inflammation affinity and radioactive diagnostic containing the same Download PDFInfo
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- AU675166B2 AU675166B2 AU75979/94A AU7597994A AU675166B2 AU 675166 B2 AU675166 B2 AU 675166B2 AU 75979/94 A AU75979/94 A AU 75979/94A AU 7597994 A AU7597994 A AU 7597994A AU 675166 B2 AU675166 B2 AU 675166B2
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K51/00—Preparations containing radioactive substances for use in therapy or testing in vivo
- A61K51/02—Preparations containing radioactive substances for use in therapy or testing in vivo characterised by the carrier, i.e. characterised by the agent or material covalently linked or complexing the radioactive nucleus
- A61K51/04—Organic compounds
- A61K51/08—Peptides, e.g. proteins, carriers being peptides, polyamino acids, proteins
- A61K51/10—Antibodies or immunoglobulins; Fragments thereof, the carrier being an antibody, an immunoglobulin or a fragment thereof, e.g. a camelised human single domain antibody or the Fc fragment of an antibody
- A61K51/1093—Antibodies or immunoglobulins; Fragments thereof, the carrier being an antibody, an immunoglobulin or a fragment thereof, e.g. a camelised human single domain antibody or the Fc fragment of an antibody conjugates with carriers being antibodies
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K51/00—Preparations containing radioactive substances for use in therapy or testing in vivo
- A61K51/02—Preparations containing radioactive substances for use in therapy or testing in vivo characterised by the carrier, i.e. characterised by the agent or material covalently linked or complexing the radioactive nucleus
- A61K51/04—Organic compounds
- A61K51/08—Peptides, e.g. proteins, carriers being peptides, polyamino acids, proteins
- A61K51/088—Peptides, e.g. proteins, carriers being peptides, polyamino acids, proteins conjugates with carriers being peptides, polyamino acids or proteins
-
- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K16/00—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies
Abstract
A peptide having affinity with inflammation is disclosed, which contains at least one of the following amino acid sequences: LLGGPS, LLGGPSV, KEYKAKVSNKALPAPIEKTISK, KEYKCKVSNKALPAPIEKTISK, KTKPREQQYNSTYR, and KTKPREQQYNSTYRVV, wherein A, C, E, G, I, K, L, N, P, Q, R, S, T, V, and Y represent amino acid residues expressed by standard one-letter symbols. According to the present invention, a peptide and its chemically modified substances, radioactive metal labeled peptides derived therefrom, and radioactive diagnostics comprising such peptide are provided, which are useful for imaging inflammation region and easy in preparation handling, and accumulate at inflammation site immediately after administration while being excellent in clearance into urine. The imaging is possible in several ten minutes after administration.
Description
I/LUU1 1 20=(1 Rogulatlan 3.2(2)
AUSTRALIA
Patents Act 1990
ORIGINAL
COMPLETE SPECIFICATION STANDARD PATENT Application Number: Lodged: f'ill" 2:I, I
IS
Invention Title: PEPTIDE HAVING INFLAMMATION AFFINITY AND RADIOACTIVE DIAGNOSTIC CONTAINING THE SAME The following statement is a full description of this invention, including the best method of performing it known to us rf 1 PEPTIDE HAVING INFLAMMATION AFFINITY AND RADIOACTIVE DIAGNOSTIC CONTAINING THE SAME The present invention relates to a peptide having affinity with inflammatory cells and its derivatives or chemically modified substances. The present invention also relates to a radioactive diagnostic useful for diagnosing inflammation sites in living body of mammals including human, which comprises the above peptide and a radioactive metal label for the peptide.
The term "inflammation" covers so-called inflammatory responses wholly, including those caused by infectious diseases or on the periphery of tumors.
Inflammation is induced by physical or chemical reactions due to heat, radiant energy, chemical substances, mechanical trauma or the like, and is also noted on infectious diseases caused by invasion into living bodies of foreign substances S" such as virus and bacteria, or on the periphery of tumors 20 resulting from, for example, mutation of DNA. Inflammation is a series of reactions initiated by reaction of tissue cells subjected to inflammatory stimuli and by subsequent reactions in microcirculation system, particularly with protein permeation through blood vessels, followed by exudation and infiltration of leukocytes and granuloma formation to healing; it may be regarded as a biological defense reaction of the i host for preventirj foreign substance from invading into the living body or fir normalizing inflammation sites.
30 Known radioactive diagnostic agents for imaging inflammations in living body including those caused by infectious diseases or on the periphery of tumors include gallium-67 citrate (Takashi Onishi, Nuclear Medicine (Kaku Igaku), Vol. 26, pp 1371-9, 1989), radioactive metal labeled polyclonal antibodies (JP-A-63502280 of Rabin. R. H et al, and Frans. H. M et al, Seminars in Nuclear Medicine, Vol 13, No.
2, April, pp 148 164, 1993), and radiolabeled leukocytes 2 (Kazuo Ito, Nuclear Medicine (Kaku Igaku), Vol. 24, pp 341 51, 1987).
Gallium-67 citrate contains gallium-67 which has a long half-life of 3.26 days, and the radioactive metal labeled polyclonal antibodies per se are also long in half-life in blood; thus both agents make the radioactive metal stay in the body for a long period of time giving unnecessary exposure to the patient. Furthermore, imaging takes 20 hours or longer with both agents. Thus, it has been impossible to get diagnostic information quickly for patients in immediate need of treatment.
Radiolabeled leukocyte diagnostic has been used in clinical practice as highly advanced medical care. However, this diagnostic requires a complicated procedure with advanced skill in which the surgeon has to prepare it by collecting blood from the patient, separating and refining leukocytes therefrom, labeling them with a radioactive metal such as 20 indium-lll and again refining them prior to administration.
This diagnostic is not prevalent because it requires a sterile room and other special equipment for preparation and thus is only usable in limited facilities In addition, the diagnostic may be hazardous to the surgeon for infection if the patient is infected by viral hepatitis, HIV or the like.
In view of the above-mentioned disadvantages of conventional compounds and their radiolabelled products such as the unnecessary exposure to patients, limitation of 30 facilities for preparation, difficulty to get image information quickly, complicated handling in preparation, and risk of infection to the operator, it is an object of the present invention to provide peptides and their chemically modified substances, radioactive metal labeled peptides derived therefrom, and radioactive diagnostics comprising such peptides, which are useful for imaging inflammation sites in living body of mammals including human, easy in preparation 3 handling, and capable of accumulating at inflammation site quickly after administration and staying there for a suitable time for imaging while being excellent in clearance into urine.
As the result of the intensive researches made by the present inventors to attain the object, peptides at least a part of which comprises a specific amino acid sequence have been found to be useful and have led to accomplishment of the present invention. One aspect of the present invention is directed to peptides having affinity with inflammation, which contain at least one amino acid sequence selected from the group consisting of
LLGGPS,
LLGGPSV,
KEYKAKVSNKALPAPIEKTISK,
KEYKCKVSNKALPAPIEKTISK,
SKTKPREQQYNSTYR,.and S. KTKPREQQYNSTYRW, 20 where A, C, E, G, I, K, L, N, P, Q, R, S, T, V, and Y represent amino acid residues expressed by standard one-letter symbols. These specific amino acid sequences hereinafter referred to as "basic amino acid sequences". Another aspect of the present invention is directed to derivatives of the above-mentioned peptides, the peptides and the derivatives labeled with radioactive metals, and radioactive diagnostics containing the peptides and/or the derivatives. Amino acid residues are expressed hereinafter by standard one- or three- Sletter symbols.
The peptides according to the present invention may be prepared by Fmoc method, a solid phase synthetic method, using a peptide synthesizer manufactured by Applied Biosystem.
The target peptide may be obtained by simultaneous deprotection and separation from resinous carrier, of the completed peptide bonded to the solid layer, followed by 4 purification with high-performance liquid chromatography (hereinafter referred to as "HPLC") utilizing a reverse phase column. The peptide may be synthesized in liquid phase or may be collected from animals or the like.
The derivatives of peptide having affinity with inflammation are those that are denatured or chemically modified so as to increase capability of accumulating at inflammatory cells, as explained hereunder. Examples of such derivatives include those in which peptides containing basic amino acid sequences are combined in parallel by use of Fmoc-K (Fmoc), those in which several peptides containing basic amino acid sequences are combined in tandem, those in which peptides containing basic amino acid sequences are combined with a bifunctional cross linking agent those in which peptides containing basic amino acid sequences are combined with a bifunctional cross linking agent an further be combined with a carrier such as polylysine or chitosan, those in which peptides are chemically modified by, for example, acetylation 20 or amidation at N-terminal and/or C-terminal, and those in which peptides are substituted with amino acids of Dconfiguration in part or as a whole.
The above-mentioned bifunctional cross linking agent is useful for increasing peptide efficacy by combining a plurality of peptides having affinity with inflammation according to the present invention to increase peptide concentration or by combining with carriers to increase the amount of peptides to be held by the carrier. Preferably, the bifunctional cross linking agent is one capable of selectively bonding to amino acid residues, including sulfosuccinimidyl 4- (N-maleimidemethyl)cyclohexane-l-carboxylate (hereinafter abbreviated as "Sulfo-SMCC"), 3-maleimidebenzoic acid Nhydroxysuccinimide ester (hereinafter abbreviated as "MBS"), N- (-maleimidecaproyloxy)succinimide (hereinafter abbreviated as "EMCS"), and succinimydyl 4-(p-maleimidephenyl)butylate 5 (hereinafter abbreviated as "SMPB"). Particularly preferable one is Sulfo-SMCC.
Preferable examples of the carrier that can combine a plurality of the peptides having affinity with inflammation include polylysine and chitosan. Chitosan is particularly preferable.
A diagnostic useful for imaging inflammation can be obtained by labeling the present peptide having affinity with inflammation or its derivatives with radioactive metal ion such as technetium-99m 99 mTc) and indium-1ll 11 1In). A bifunctional ligand is conveniently used for labeling with radioactive metal ion. Preferable examples of the ligand include diethylenetriamine pentaacetic acid (hereinafter abbreviated as "DTPA"), ethylenediaminetetraacetic acid (hereinafter abbreviated as "EDTA"), and 1,4,7,10tetraazacyclododecane-l-aminoethylcarbamoylmethyl-4,7,10tris[(R,S)-methylacetic acid] (hereinafter abbreviated as 20 "DO3MA"). DTPA is most preferable.
Alternatively, labeling with a radioactive metal may be carried out by dissolving the present peptide or a derivative thereof in a physiological saline, an aqueous buffer solution or the like and allowing it to react with a radioactive metal. In case of technetium-99m, a peptide can be labeled by an ordinary process wherein a reduction agent having a proper redox potential such as stannous chloride is added to the peptide, followed by mixing with a sodium 30 pertechnetate solution. In case of indium-1ll, a peptide can be labeled by mixing the peptide with a weak acidic aqueous solution containing indium-1ll ions. If required, unreacted pertechnetate ions or indium-1ll ions may be removed by HPLC or other means.
Furthermore, the present diagnostic may be provided in a form of a kit so that it can be prepared as required.
6 The kit may include a pharmaceutically acceptable stabilizer such as ascorbic acid or p-aminobenzoic acid, a pH adjusting agent such as an aqueous buffer solution, an excipient such as D-mannitol, and an agent useful for improving radiochemical purity such as tartaric acid, or malonic acid.
Pharmaceutically acceptable peptide compounds comprising a peptide containing a radioactive metal in accordance with the present invention efficiently accumulate at inflammation sites just after generally-employed parenteral administration such as intraveous bolus injection, attain quick distribution of the radioactive substance, provide a target site/background ratio sufficient to complete imaging within one hour after administration, and stay at the target site for a suitable period of time for imaging and thereafter are quickly excreted into urine via kidney; all of these features are desirable for a diagnostic. Thus, the peptide has excellent characteristics for overcoming conventional problems while enabling a diagnosis to be made by use of a radioactive imaging apparatus that is generally available.
The present radioactive diagnostic comprising the peptide having affinity with inflammation can be administered parenterally in accordance with a common practice such as intraveous bolus injection; the amount of administration is decided so as to obtain a radiation dose sufficient for imaging in consideration of various conditions such as weight and age of the patient as well as type of radioactive imaging apparatus. In case of human, a radiation dose from 185 to 30 1110 MBq us usually preferable.
Now, examples of the peptide having affinity with inflammation and its derivative according to the present invention are shown hereunder.
7
DTPA
KGGPELLGGPSV
DTPA
(Formula 1)
CGCGGLLGGPSV
(Formula 2) C(Acm)GC(Acm)GGPELLGGPSVPEJ
LLGGPSVPELLGGPSVA
(Formula 3)
PELLGGPSV
PELLGGPSV
PELLGGPSV
PELLGGPSV
"K
PELLGGPSV
!(Acm)GC(Acm) (Formula 4) (LLGGPSVC-Sulfo SMCC)xCHI(DTPA)y where x y 5 (Formula Now, the present invention is illustrated in more details by way of examples and the drawings in which FIG. 1 is a whole body scintigram of an inflammation model rat one hour after administration of radioactive metal labeled Peptide-4; FIG. 2 is a whole body scintigram of an inflammation model rat one hour after administration of radioactive metal labeled FIG. 3 is a whole body scintigram of an inflammation model rat one hour after administration of radioactive metal labeled Peptide-6; and 8 FIG. 4 is a whole body scintigram of a model rat with infectious disease one hour after administration of radioactive metal labeled Peptide-6.
While the technetium-99m labeling was made in the examples according to the process described in WO-A-92/13572, the object of the example is to prove that the peptide according to the present invention is able to image inflammation sites without change in performance regardless of kinds of nuclide or labeling method.
EXAMPLE 1 SYNTHESIS OF KGGPELLGGPSV (Peptide-1) Synthesis was made with Peptide Synthesizer (Model 431A) manufactured by Applied Biosystems using HMP Resin by Fmoc process under 0.25 mM scale condition. Excision of the peptide was made by a reaction for 2.5 hours in aqueous 95 trifluoroacetic acid (hereinafter abbreviated as "TFA") 20 containing 2.5 ethanedithiol (hereinafter abbreviated as Purification was made by HPLC under the following conditions: Column: YMC-PackR&D--ODS-5-ST (4.6 x 150 mm) Elution velocity: 6 mL/min Eluent A: 0.1 TFA/purified water Eluent B: 0.1 TFA/acetonitrile Concentration gradient: 0 min (10 B) 15 min (20 B) 40 min (50 B) 30 Then, PICO-TAG-TM-Workstation manufactured by Waters was used for identifying the amino acid composition corresponding to the main peak. After it was confirmed that the composition was of the target peptide, the peak coinciding with the amino acid composition was freeze-dried to yield 59.6 mg of the lyophilized product. The analytical value (number per molecule) for the amino acid composition of the product 9 peptide is shown below together with the theoretical value in parentheses: Ser:1.3 Gly:4.4 Pro:2.0 Val:1.1 Leu:2.1 Lys:1.2 For the purpose of confirming the reliability of the Peptide Synthesizer, the amino acid sequence of the product peptide was determined by Protein Sequencer (a peptide automatic analyzer) Model 477A manufactured by Applied Biosystems. In addition, C-terminal analysis was made for confirming the C-terminal. As a result, the sequence from the N-terminal to S at the eleventh position coincided with the target sequence. The C-terminal analysis showed that the Cterminal was V. Thus, the peptide was confirmed to have an amino acid sequence of KGGPELLGGPSV.
EXAMPLE 2 SYNTHESIS OF CGCGGLLGGPSV (Peptide-2) 20 Synthesis was made by the method described in EXAMPLE 1. Purification was made by HPLC under the following conditions: Column: YMC-PackR&D--ODS-5-ST (4.6 x 150 mm) S'Elution velocity: 1 mL/min Eluent A: 0.1 TFA/purified water Eluent B: 0.1 TFA/acetonitrile Concentration gradient: 0 min (5 B) 40 min (30 B) 120 min (60 B) 30 After the amino acid composition corresponding to the main peak is determined in the same way as EXAMPLE 1 to confirm that the target peptide was obtained, the peak obtained was freeze-dried to yield 20 mg of the lyophilized product. The analytical value (number per molecule) for the amino acid composition of the product peptide is shown below together with the theoretical value in parentheses: 10 Gly:4.9 Pro:1.0 Val:1.0 Cys:0.9 Leu:2.0 EXAMPLE 3 SYNTHESIS OF LLGGPSVC (Peptide-3) A peptide having LLGGPSVC amino acid sequence was synthesized in an amount of 25 mg according to tne method described in EXAMPLE 1, and the peptide was analyzed for the amino acid composition. The analytical value (number per molecule) for the amino acid composition of the product peptide is shown below together with the theoretical value in parentheses: Ser:0.9 Gly:2.0 Val:1.0 Leu:1.8 Pro:1.0 Cys:1.2 EXAMPLE 4 SYNTHESIS OF C(Acm)GC(Acm)GGGKEYKAKVSNKALPAPIEKTISK (Peptide-4) S" 20 Synthesis Was made by the method described in EXAMPLE 1. Acm (acetamide methyl group) is a protective group for -SH group in cysteine. Excision of the peptide was made by allowing 100 mg of the resultant compound to react for 2.5 hours in 10 ml of aqueous solution in which 0.25 ml of EDT, 0.75 g of crystalline phenol, 0.5 ml of thioanisole, 0.5 ml of purified water and 9.5 ml of TFA were mixed. Purification was made by HPLC under the following conditions: Column: YMC-PackR&D-ODS-5-ST (20 x 150 mm) Elution velocity: 8 mL/min 30 Eluent A: 0.1 TFA/purified water Eluent B: 0.1 TFA/acetonitrile Concentration gradient: 0 min (10 B) -k 15 min (15 B) 40 min (50 B) After the amino acid composition corresponding to the main peak is determined in the same way as EXAMPLE 1 to confirm that the target peptide was obtained, the peak coinciding with 11 the _iino acid composition was freeze-dried to yield 45 mg of the lyophilized product with purity of 95 or more. Since C(Acm) is unable to be identified by PICO-TAG method, the presence of C(Acm)GC(Acm) was confirmed by technetium-99m labeling. The analytical value (number per molecule) for the amino acid composition of the product peptide is shown below together with the theoretical value in parentheses: Asn:1.1 Glu:2.0 Ser:2.3 Gly:4.4 Thr:l.0 Ala:3.2 Pro:2.1 Tyr:0.6 Val:0.9 Ile:2.8 Leu:1.3 Lys:5.7 Cys: The amino acid sequence of the resulting peptide was determined using the same Sequencer as EXAMPLE 1; the sequence from the N-terminal to the 26th residues coincided with the target sequence. Thus, the peptide was confirmed to have an amino acid sequence of C(Acm)GC(Acm)GGGKEYKAKVSNKALPAPIEKTISK.
EXAMPLE 20 SYNTHESIS OF C(Acm)GC(Acm)GGKTKPREQQYNSTYRVV Synthesis was made by the method described in EXAMPLE 1. Excision of the peptide was made by allowing 15 r mg of the resultant compound to react for 1.5 hours in 10 r, of aqueous solution in which 0.25 ml of EDT, 0.75 g of crystalline phenol, 0.5 ml of thioanisole, 0.5 ml of purified water and 9.5 ml of TFA were mixed. Purification was made by HPLC under the following conditions: Column: YMC-PackR&D--ODS-5-ST (20 x 150 mm) S" 30 Elution velocity: 8 mL/min Eluent A: 0.1 TFA/purified water Eluent B: 0.1 TFA/acetonitrile Concentration gradient: 0 min (10 B) 15 min (10 B) 90 min (40 B) Then, using the same analysis unit as EXAMPLE 1, the amino acid composition corresponding to the main peak was 12 identified. After it was confirmed that e composition was of the target peptide, the peak coinciding with the amino acid composition was freeze-dried to yield 51 mg of the lyophilized product of which purity was not less than 95 The analytical value (number per molecule) for the amino acid composition of the product peptide is shown below together with the theoretical value in parentheses: Asp:l.l Glx:3.1 Ser:1.0 Gly:3.3 Arg:2.1 Thr:2.2 Pro:l.l Tyr:1.2 Val:1.7 Cys: Lys:5.9 (6) EXAMPLE 6 SYNTHESIS OF (PELLGGPSV) x 4 in parallel x 2 in parallel (KGGC(Acm)GC(Acm)) (Peptide-6) Synthesis was made by the method described in EXAMPLE 1. Purification was made by HPLC under the following conditions: 20 Column: YMC-PackR&D.-ODS-5-ST (20 x 150 mm) Elution velocity: 8 mL/min Eluent A: 0.1 TFA/purified water Eluent B: 0.1 TFA/acetonitrile Concentration gradient: 0 min (15 B) 15 min (15 B) 100 min (60 B) Then, using the same analysis unit as EXAMPLE 1, the amino acid composition corresponding to the main peak was identified. After it was confirmed that the composition was 30 of the target peptide, the peak coinciding with the amino acid composition was freeze-dried to yield 22.1 mg of the lyophilized product. The analytical value (number per molecule) for the amino acid composition of the product peptide is shown below together with the theoretical value in parentheses: Glu:3.9 Ser:4.1 Gly:11.8 Pro:7.9 Val:2.9 Leu:7.6 Lys:2.1 Cys: (2) 13 EXAMPLE 7 SYNTHESIS OF C(Acm)GC(Acm)GGr(PELLGGPSV) x 3 repeats in tandemIA (Peptide-7) Synthesis was made by the method described in EXAMPLE 1. Purification was made by HPLC under the following conditions: Column: YMC-PackR&D-ODS-5-ST (20 x 150 mm) Elution velocity: 8 mL/min Eluent A: 0.1 TFA/purified water Eluent B: 0.1 TFA/acetonitrile Concentration gradient: 0 min (15 B) 15 min (15 B) 100 min (60 B) Then, using the same analysis unit as EXAMPLE 1, the amino acid composition corresponding to the main peak was identified. After it was confirmed that the composition was of the target peptide, the peak coinciding with the amino acid composition was freeze-dried to yield 55.6 mg of the lyophilized product. The analytical value (number per molecule) for the amino acid composition of the product peptide is shown below together with the theoretical value in parentheses: Glu:3.1 Ser:3.0 Gly:9.7 Pro:6.9 Val:2.9 Leu:6.0 Ala:2.0 (1) e*e 0 30 o *e* EXAMPLE 8 INTRODUCTION OF BIFUNCTIONAL LIGAND (DTPA) INTO LYSINE RESIDUE OF Peptide-1 Peptide-1 obtained in EXAMPLE 1, in an amount of [imol, was dissolved in 3.0 ml of a 0.1 M phosphate buffer solution (pH 10 times volume of DTPA anhydride was added to the mixture with agitation at room temperature and allowed to react for 30 minutes. Three peaks were obtained from the 14 mixture by HPLC separation using 230 nm detection wavelength.
Indium-111 was labeled to each of the peak components for determining the target peak; the labeling ratio was determined by electrophoresis using acethylcellulose membrane.
Radiochemical purity was 96.0 for peak 1, 98.0 for peak 2, and 38.0 for peak 3. The high labeling ratio of 98.0 for the peak 2 component led to the conclusion that this component was the target compound having the bifunctional ligand combined to the peptide. The peak 2 component was freeze-dried to yield 7.1 mg of the DTPA combined peptide.
EXAMPLE 9 INTRODUCTION OF BIFUNCTIONAL LIGAND (DTPA) INTO CHITOSAN- PENTAMER (CHI-PENTAMER) Chitosan-pentamer, in an amount of 32.8 [imol, was dissolved in 3.0 ml of a 0.1 M bicarbonate buffer solution (pH 5 times volume of DTPA anhydride was added to the mixture with agitation at room temperature and allowed to react for 1 hour. The mixture solution was refined by electrodialysis for 2.5 hours using the unit (Micro Acilyzer Sl) of Asahi Chemical Industry Co., Ltd. The resultant sample was analyzed quantitatively by ninhydrine reaction of the "unreacted primary amines. The analysis showed the presence of at least two unreacted primary amines, indicating from 1 to 3 DTPAs were introduced into the CHI-pentamer.
EXAMPLE SYNTHESIS OF Peptide-3-Sulfo-SMCC-CHI-pentamer-DTPA DTPA-CHI-pentamer obtaired in EXAMPLE 9, in an amount of 10 nmol, was dissolved in 8.0 ml of a 50 mM borate buffer solution (pH 50 nmol of Sulfo-SMCC was added to the aqueous solution with agitation at 30 OC and the mixture was allowed to react for 1 hour. Purification was made by 15 electrodialysis using the unit of Asahi Chemical Industry Co., Ltd. followed by dry-freezing. A 37.5 portion of the product compound was aliquoted and dissolved into a 0.1 M tris-HCl buffer solution (pH To this mixture, 12 pmol of Peptide-3 obtained in EXAMPLE 3 was added; the whole was allowed to react in a low temperature room overnight, then concentrated and purified by HPLC. Two peaks were obtained using 215 nm detection wavelength (retention time: 61 minutes for peak 1, and 73 minutes for peak Indium-111 was labeled to each of the peak components, and radiochemical purity was determined by electrophoresis; peak 1 was 82.6 and peak 2 was 83.4 Since hydrophobicity of the whole compound increases as the number of the peptides combined to CHI increases, further experiments were made using the peak 2 that appeared to be the target compound because of the longer HPLC retention time.
EXAMPLE 11 N-TERMINAL ACETYLATION OF KGGPELLGGPSV (Peptide-1) An amount of 8.0 mol of Peptide-1 prepared in EXAMPLE 1 was dissolved in 1.0 mL of a 0.3 M phosphate buffer solution (pH 20 tl of acetic anhydride was added thereto with agitation at 4 OC and the mixture was allowed to react S 25 for 12 hours. After the completion of reaction, the N- S* terminal acetylation was checked by measuring absorbance at a wavelength of 570 nm. Result was 1.734 for N-terminal amine and 0.249 for N-terminal acetylated, which means that 85.7 was acetylted. It is known that as combination of acetyl 30 group to N-terminal increases, the hydrophobicity of the peptide and retention time are extended upon reverse-phase HPLC. On this basis, the HPLC analysis was conducted and indicated that the retention time was 13.72 minutes for the starting peptide-1, and 14.93 minutes for the N-terminal acetylated peptide-1. The extension of about one minute of the retention time verified the acetylation of the N-terminal of the peptide.
16 EXAMPLE 12 C-TERMINAL AMIDATION AND N-TERMINAL ACETYLATION OF C(Acm)GC(Acm'GGGKEYKAKVSNKAIPAPIEKTISK (Peotide-4) In the process described in EXAMPLE 1, PAL (Peptide Amide Linker) Resin made by MILLIPORE was used in place of the HMP Resin to synthesize C(Acm)GC(Acm)GGGKEYKAKVSNKALPAPIEKTISK of which C-terminal was amidated. Then, its N-terminal was acetylated by acetic anhydride using N-hydroxybenzotriazole (HOBt) as an activation agent.
Excision of the peptide was made by allowing 150 mg of the resultant compound to react for 2 hours in 10 ml of aqueous solution in which 0.25 ml of EDT, 0.75 g of crystalline phenol, 0.5 ml of thioanisole, 0.5 ml of purified water and 9.5 ml of TFA were mixed. Purification was made by HPLC under the following conditions: Column: YMC-PackR&D-ODS-5-ST (20 x 150 mm) Elution velocity: 8 mL/min Eluent A: 0.1 TFA/purified water Eluent B: 0.1 TFA/acetonitrile Concentration gradient: 0 min (10 B) 15 min (15 B) 75 min (50 B) r Then, using the same analysis unit as EXAMPLE 1 for analyzing the amino acid composition, the amino acid composition corresponding to the resultant main peak was identified. After it was confirmed that the composition was of the target peptide, the peak coinciding with the amino acid composition was freeze-dried to yield 32 mg of the lyophilized product of which purity was not less than 95 The analytical value (number per molecule) for the amino acid composition of the product peptide is shown below together with the theoretical value in parentheses: 17 Asn:l.l Glu:2.1 Ser:2.0 Gly:3.8 Thr:l.l Ala:3.1 Pro:2.1 Tyr:0.6 Val:1.0 Cys: Ile:2.2 Leu:1.2 Lys:5.9 (6) EXAMPLE 13 C-TERMINAL AMIDATION AND N-TERMINAL ACETYLATION OF C(Acm)GC(Acm)GGKTKPREQQYNSTYRVV In the process described in EXAMPLE 1, PAL Resin manufactured by MILLIPORE was used in place of the HMP Resin to synthesize C(Acm)GC(Acm)GGKTKPREQQYNSTYRVV of which Cterminal was amidated. Then, its N-terminal was acetylated by acetic anhydride using N-hydroxybenzotriazole (HOBt) as an activation agent.
Excision of the peptide was made by allowing 150 mg of the resultant compound to react for 1.5 hours in 10 ml of aqueous solution in which 0.25 ml of EDT, 0.75 g of crystalline phenol, 0.5 ml of thioanisole, 0.5 ml of purified water and 9.5 ml of TFA were mixed. Purification was made by HPLC under the following conditilos: Column: YMC-PackR&D-ODS-5-ST (20 x 150 mm) Elution velocity: 8 mL/min Eluent A: 0.1 TFA/purified water S: 25 Eluent B: 0.1 TFA/acetonitrile Concentration gradient: 0 min (10 B) 15 min (10 B) 75 min (50 B) Then, using the same analysis unit as EXAMPLE 1 for 30 analyzing the amino acid composition, the amino acid S composition corresponding to the resultant main peak was identified. After it was confirmed that the composition was the target peptide, the peak coinciding with the amino acid composition was freeze-dried to yield 23 mg of the lyophilized product of which purity is not less than 95 The analytical value (number per molecule) for the amino acid composition of 18 the product peptide is shown below together with the theoretical value in parentheses: Asp:l.l Glx:3.2 Ser:0.9 Gly:3.1 Arg:2.2 Thr:2.2 Pro:l.l Tyr:1.3 Val:1.6 Cys: Lys:5.9 (6) EXAMPLE 14 PREPARATION OF INDIUM-111 LABELED PEPTIDE Peptide-1-DTPA obtained in EXAMPLE 8, in an amount of 100 through 200 nmol was adjusted to pH 5.7 in a 0.1 M citrate buffer solution, and then 37 to 74 MBq of indium 111 In) chloride was added thereto. After agitation, the solution was left as such for 15 minutes. A part of the solution was taken and checked for the labeling percentage by electrophoresis. The radiochemical purity of the target compound was 98 Peptide-3-Sulfo-SMCC-CHI-DTPA obtained in EXAMPLE 10 was also labeled with In-ill in the same way as above, and the radiochemical purity of the target compound was 90 EXAMPLE TECHNETIUM-99m LABELING OF PEPTIDES CONTAINING CGC SEQUENCE An amount of 240 300 nmol of Peptide-2 obtained in EXAMPLE 2 was taken into each vial, and a volume of a 0.1 M phosphate buffer solution (pH 8.0) was added thereto to adjust the whole molarity to 300 pmol. Atmosphere in the vial was replaced with argon; then 180 300 nmol of dithiothreitol was added thereto. The mixture was then allowed to react for one hour at room temperature. Next, 120 nmol of stannous chloride and 740 1110 MBq of sodium pertechnetate were added. The mixture was left for one hour under gentle agitation.
Peptide-2 labeled with technetium-99m was yielded. Peptide labeled had radiochemical purity not less than 90 19 EXAMPLE 16 PREPARATION OF GLUCOHEPTANATE LABELED WITH TECHNETIUM-99m An amount of 20.4 cmol of glucoheptanic acid was dissolved into a 0.1 M phosphate buffer solution (pH 8.0) to adjust the total volume to 450 Atmosphere in the vial was replaced with argon; then 120 imol of stannous chloride and 2.2 GBq of sodium pertechnetate were added. The mixture was gently agitated for 30 minutes. Thereby, glucoheptanate labeled with technetium-99m was yielded.
EXAMPLE 17 TECHNETIUM-99m LABELING OF PEPTIDES CONTAINING C(Acm)GC(Acm)
,EQUENCE
Experiments were made for all the peptides those prepared in EXAMPLEs 4, 5, 6 and 7. Each of the peptides was taken, in an amount of 0.2 1.0 pmol, into a vial respectively, and a volume of a 0.1 M phosphate buffer solution (pH 8.0) was added thereto to adjust the whole volume to 500 Jl. Atmosphere in the respective vial was replaced with argon. To each vial, 500 ul of 1.5 2.2 GBq/ml glucoheptanate labeled with technetium-99m yielded in EXAMPLE 16 was added and quickly agitated. Thereafter, the mixture was allowed to react for 20 minutes in a boiling water bath.
Labeling percentage of all the experimented peptides after cooling was 90 95 according to TLC.
EXAMPLE 18 IMAGING OF INFLAMMATION SITES USING INDIUM-111 LABELED PEPTIDE To the right femoral part of Sparague-Davley Rats S" weighing about 220 g, 100 p1 of turpentine oil was subcutaneously administered. After 24 hours, when inflammation was clearly observed, Ravonal anesthesia was applied; then, Peptide-l-DTPA-indium-111 and Peptide-3-Sulfo- C
L
20 SMCC-CHI-DTPA-indium-111 obtained in EXAMPLE 14 were respectively administered in an amount of 3.7 MBq 7.4 MBq to the respective tail vein. Images were obtained with gamma camera one, three, and six hours later. A site of interest was set on the image, where the ratio ratio) of total counts for the inflammation site to total counts for the corresponding normal site of the opposite leg was determined. The ratio, one hour after the administration, was 2.63 for Peptide-l-DTPA-indium-111 and 2.09 for Peptide-3-DTPA-indium-lll, whereby the focal site was evidently imaged. Table 1 shows time course of the ratios (mean value standard error) for three rats with respective peptides.
Table 1 ratio of In-ill labeled peptides in inflammation model rats Labeled Period of time after administration Peptide 1 hr. 3 hrs. 6 hrs.
Peptide-1 2.63 0.19 2.30 0.13 1.71 0.18 Peptide-3 2.09 0.18 2.46 0.29 2.78 0.15 s r EXAMPLE 19 IMAGING OF INFLAMMATION SITES USING TECHNETIUM-99m LABELED
PEPTIDE
After Ravonal anesthesia was applied to the model rats described in EXAMPLE 18, 37 74 MBq of technetium-99m labeled Peptide-2 obtained in EXAMPLE 15, Peptide-4, Peptide- Peptide-6 and Peptide-7 obtained in EXAMPLE 17 were each administered to the respective tail vein. Images were obtained with gamma camera 30 minutes and one, three, and six hours later respectively. A site of interest was set on the image and the ratio was determined. The ratio, one hour after the administration, was 3.35 for Peptide-2, 4.98 for Peptide-6, 3.36 for Peptide-7, 4.27 for 21 Peptide-4 and 4.41 for Peptide-5 whereby the focal sie was evidently imaged. Table 2 shows time course of the ratios (mean value standard error) for three rats with respective peptides.
Table 2 ratio of Tc-99m labeled peptide in inflammatory model rats Labeled Period of time after administration Peptide 30 mins 1 hr. 3 hrs. 6 hrs.
Peptide-2 3.35 0.33 2.78 0.23 2.82 0.17 Peptide-4 2.47 0.17 4.27 0.26 3.10 0.20 2.61 0.08 4.41 0.62 3.85 0.63 Peptide-6 4.98 0.23 4.61 0.49 3.20 0.39 Peptide-7 3.36 0.31 2.18 0.39 2.26 0.20 oo 0 o o oo o f ooo ftee ftfof ft f t ft ft f ft ft g* ft: fto oft ft ft ftf EXAMPLE IMAGING OF RAT MODEL WITH INFECTIOUS DISEASE USING TECHNETIUM- 99m LABELED PEPTIDE In 1.0 mL of physiological saline, 108 of viable microbe cells of Staphylococcus aureus were suspended. An aliquot of 100 p.l was administered intramuscularly to the 25 right femoral region of Sparague-Davely Rats weighing about 220 g. After 24 hours, Ravonal anesthesia was applied to the model rats that had clearly evident inflammation; then, 37 74 MBq of technetium-99m labeled Peptide-6 obtained in EXAMPLE 8 was administered to the tail vein. Images were obtained 30 with gamma camera one, three, and six hours later respectively. A site of interest was set on the image, and the ratio was determined. One hour after the administration, the ratio showed 1.92 indicating that focal region was evidently imaged. Table 3 shows time course of the ratios (mean value standard error) with this peptide.
22 Table 3 ratio of Tc-99m labeled peptide in model rats with infectious disease Labeled Period of time after administration Peptide 1 hr. 3 hrs. 6 hrs Peptide-6 1.92 0.10 1.58 0.05 1.52 0.17 EXAMPLE 21 SAFETY OF THE PEPTIDES Assuming that clinical dosage to human is 1.0 kg, bolus administration of Peptide-1, Peptide 4 and in an amount of 8.3 ptg per 1.0 g of rat and physiological saline as control were made respectively to the tail vein of the rat. Immediately after the administration, behavior of the rat was observed. The observation was continued until five days later; zero minute, ten minutes, three hours, six hours, one day, two days, three days, four days, and five days later. Just after the peptide administration, symptoms such as slobber, vomiting, ocular proptosis, and behavioral abnormality were not observed. Furthermore, extreme change in weight, weight gain or loss was not observed until five days later. After weighing five days later, the rats were 25 dissected. Abnormality in tissue was checked with the naked eye; abnormality in any tissue was not noted such as hemostatis, pigmentation, or discoloration. These gave estimation that more than 1,000 times administration of the assumed clinical dosage would be safe.
As explained, the present invention provides a peptide and its chemically modified substances, radioactive S metal labeled peptides derived therefrom, and radioactive diagnostics comprising such peptide, which are useful for imaging inflammation sites in living body of mammals including human and easy in preparation handling, and accumulate at inflammation sites immediately after the administration and 23 stay there for a time suitable for imaging while being excellent in clearance via kidney into urine; thereby eliminating unnecessary exposure to patients, limitation of facilities for preparation, difficulty to get image information quickly, complicated handling and skill in preparation, and risk of infection to the operator. According to the present invention, the imaging is possible in several ten minutes after administration.
0 ft 4 oo o W o °*ee «o 0 *oe o8 *e•
Claims (12)
1. A peptide having affinity with inflammation, which cemprises at least one of the following amino acid sequences: LLGGPS, LLGGPSV, KEYKAKVSNKALPAPIEKTISK, KEYKCKVSNKALPAPIEKTISK, KTKPREQQYNSTYR, and KTKPREQQYNSTYRVV, wherein A, C, E, G, I, K, L, N, P, Q, R, S, T, V, and Y represent amino acid residues expressed by standard one-letter symbols.
2. A peptide derivative having affinity with inflammation, which comprises the peptide of Claim 1 combined with a bifunctional cross linking agent.
3. A peptide derivativc having affinity with inflammation, which comprises the peptide of Claim 1 combined with a bifunctional ligand.
4. A peptide derivative having affinity with 25 inflammation, which comprises the peptide of claim 2 combined with a carrier through the bifunctional cross linking agent.
A peptide derivative having affinity with inflammation according to Claim 4, in which a bifunctional 30 ligand is combined with the carrier. o*
6. A peptide derivative having affinity with inflammation according to Claim 2, 4 or 5, wherein the bifunctional cross linking agent is one selected from the group consisting of sulfosuccinimidyl 4-(N-maleimidemethyl) cyclohexane-1-carboxylate, 3-maleimidebenzoic acid N- i hydroxysuccinimide ester, N-(e-maleimidecaproyloxy) succinimide, and succinimydyl 4-(p-maleimidephenyl) butylate.
7. A peptide having affinity with inflammation according to Claim 3, wherein the bifunctional ligand is one selected from the group consisting of diethylenetriamine pentaacetic acid, ethylenediaminetetraacetic acid, and 1,4,7,10-tetraazacyclododecane-1 -aminoethylcarbamoylmethyl-4,7,1 0-tris [(R,S)-methylacetic acid].
8. A peptide derivative having affinity with inflammation according to Claim wherein the bifuncational ligand is one selected from the group consisting of diethylenetriamine pentaacetic acid, ethylenediaminetatraacetic acid, and 1,4,7,10-tetraazacyclododecane-l-aminoethylcarbamoylmethyl 1-4,7,10-tris [(R,S)-methylacetic acid].
9. A peptide derivative having affinity with inflammation according to Claim 4 or 5, wherein the carrier is polylysine or chitosan.
10. A peptide labelled with a radioactive metal, which comprises the peptide or its derivative of Claim 1, 3, 5, 7 or 8 with which a radioactive metal ion is coordinated.
11. A peptide labelled with a radioactive metal according to Claim wherein the radioactive metal ion is technetium-99m or indium-111.
12. A radioactive diagnostic comprising the radioactive metal labelled peptide of Claim 10 or 11. DATED this 29th day of October, 1996 NIHON MEDI-PHYSICS CO LTD WATERMARK PATENT TRADEMARK ATTORNEYS 290 BURWOOD ROAD HAWTHORN VICTORIA 3122 AUSTRALIA SI 26 ABSTRACT A peptide having affinity with inflammation is disclosed, which contains at least one of the following amino acid sequences: LLGGPS, LLGGPSV, KEYKAKVSNKALPAPIEKTISK, KEYKCKVSNKALPAPIEKTISK, KTKPREQQYNSTYR, and KTKPREQQYNSTYRW, wherein A, C, E, G, I, K, L, N, P, Q, R, S, T, V, and Y represent amino acid residues expressed by standard one-letter symbols. According to the present invention, a peptide and its chemically modified substances, radioactive metal labeled peptides derived therefrom, and radioactive diagnostics comprising such peptide are provided, which are useful for imaging inflammation region and easy in preparation handling, and accumulate at inflammation site immediately after 20 administration while being excellent in clearance into urine. The imaging is possible in several ten minutes after administration. S S *o o *oeo
Applications Claiming Priority (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| JP28775293 | 1993-10-22 | ||
| JP5-287752 | 1993-10-22 |
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| Publication Number | Publication Date |
|---|---|
| AU7597994A AU7597994A (en) | 1995-05-11 |
| AU675166B2 true AU675166B2 (en) | 1997-01-23 |
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| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| AU75979/94A Ceased AU675166B2 (en) | 1993-10-22 | 1994-10-20 | Peptide having inflammation affinity and radioactive diagnostic containing the same |
Country Status (9)
| Country | Link |
|---|---|
| US (1) | US5821330A (en) |
| EP (1) | EP0649857B1 (en) |
| KR (1) | KR100316376B1 (en) |
| AT (1) | ATE175976T1 (en) |
| AU (1) | AU675166B2 (en) |
| CA (1) | CA2134051A1 (en) |
| DE (1) | DE69416078T2 (en) |
| DK (1) | DK0649857T3 (en) |
| ES (1) | ES2126695T3 (en) |
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| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US5989519A (en) * | 1992-03-13 | 1999-11-23 | Diatide, Inc. | Technetium-99m labeled peptides for imaging inflammation |
| WO1993017719A1 (en) * | 1992-03-13 | 1993-09-16 | Diatech, Inc. | TECHNETIUM-99m LABELED PEPTIDES FOR IMAGING INFLAMMATION |
| CA2165228A1 (en) * | 1994-12-27 | 1996-06-28 | Yoshitoshi Itaya | Metal chelate forming peptides and use thereof |
| DE19514088A1 (en) * | 1995-04-13 | 1996-10-17 | Deutsches Krebsforsch | Conjugate for the treatment of inflammation, infection and / or skin diseases |
| AU757554B2 (en) * | 1998-02-11 | 2003-02-27 | Bracco International B.V. | Angiogenesis targeting molecules |
| WO2001052898A1 (en) * | 2000-01-21 | 2001-07-26 | Mallinckrodt Inc. | Methods for incorporating metal chelators at carboxyl-terminal site of peptides |
| AU2001236485A1 (en) * | 2000-01-21 | 2001-07-31 | Mallinckrodt, Inc. | Novel orthogonally protected amino acid chelators for biomedical applications |
| AU2001234478A1 (en) * | 2000-01-21 | 2001-07-31 | Mallinckrodt, Inc. | Chelating agents and method for their use as tandem metal chelators and hydrophilic spacers for medical diagnosis and therapy |
| EP2279757A3 (en) | 2000-06-02 | 2011-08-03 | Bracco Suisse SA | Compounds for targeting endothelial cells |
| US8263739B2 (en) | 2000-06-02 | 2012-09-11 | Bracco Suisse Sa | Compounds for targeting endothelial cells, compositions containing the same and methods for their use |
| KR100882751B1 (en) * | 2002-05-08 | 2009-02-09 | 재단법인서울대학교산학협력재단 | Oligopeptide which binds specifically to chitosan |
| TW200505934A (en) * | 2003-03-26 | 2005-02-16 | Nihon Mediphysics Co Ltd | Compound having affinity with calcified tissue |
Citations (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US5363846A (en) * | 1986-01-16 | 1994-11-15 | The General Hospital Corporation | Method for the diagnosis and treatment of inflammation |
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| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| JPS62153300A (en) * | 1985-12-26 | 1987-07-08 | Teijin Ltd | Fc region protein of human immunoglobulin g and production thereof |
| WO1987004351A1 (en) * | 1986-01-16 | 1987-07-30 | The General Hospital Corporation | Method for the diagnosis and treatment of inflammation |
| AU593611B2 (en) * | 1986-02-14 | 1990-02-15 | Nihon Medi-Physics Co., Ltd. | High molecular compounds having amino groups, and their utilization |
| EP0584421A1 (en) * | 1992-08-21 | 1994-03-02 | Cécile Casterman | Immunoglobulins devoid of light chains |
-
1994
- 1994-10-20 DE DE69416078T patent/DE69416078T2/en not_active Expired - Fee Related
- 1994-10-20 ES ES94116583T patent/ES2126695T3/en not_active Expired - Lifetime
- 1994-10-20 DK DK94116583T patent/DK0649857T3/en active
- 1994-10-20 AT AT94116583T patent/ATE175976T1/en active
- 1994-10-20 EP EP94116583A patent/EP0649857B1/en not_active Expired - Lifetime
- 1994-10-20 AU AU75979/94A patent/AU675166B2/en not_active Ceased
- 1994-10-21 CA CA002134051A patent/CA2134051A1/en not_active Abandoned
- 1994-10-21 US US08/327,459 patent/US5821330A/en not_active Expired - Fee Related
- 1994-10-22 KR KR1019940027150A patent/KR100316376B1/en not_active IP Right Cessation
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| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US5363846A (en) * | 1986-01-16 | 1994-11-15 | The General Hospital Corporation | Method for the diagnosis and treatment of inflammation |
Also Published As
| Publication number | Publication date |
|---|---|
| DK0649857T3 (en) | 1999-09-13 |
| ATE175976T1 (en) | 1999-02-15 |
| KR950011467A (en) | 1995-05-15 |
| AU7597994A (en) | 1995-05-11 |
| DE69416078D1 (en) | 1999-03-04 |
| KR100316376B1 (en) | 2002-02-19 |
| EP0649857A1 (en) | 1995-04-26 |
| EP0649857B1 (en) | 1999-01-20 |
| US5821330A (en) | 1998-10-13 |
| CA2134051A1 (en) | 1995-04-23 |
| DE69416078T2 (en) | 1999-05-27 |
| ES2126695T3 (en) | 1999-04-01 |
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